Knowledge of gametogenesis and structure of mature gametes is important for understanding the reproductive
biology of a species under study. Among phoronids, Phoronis embryolabi is distinguished by a most unusual type
of development: larval viviparity. In the present work, we characterize spermatogenesis in this species using
transmission and scanning electron microscopy. The results indicate that the development of male gametes
occurs within the vasoperitoneal tissue. Early spermatocytes have a well-developed secretory apparatus
comprising a Golgi body and endoplasmic reticulum. The Golgi body, which is retained until the late spermatid
stage, produces acrosome material, thick glycocalyx, and membrane vesicles that are presumably necessary for
the elongation of initially small cells into filiform mature spermatozoa. The germ cells retain their connections
with each other until the late spermatid stage. The mature sperm of P. embryolabi can be regarded as an introsperm,
which is characteristic of species with internal fertilization. The structure of mature sperm differs from
that of other phoronid species, whose sperm can be described in terms of the form and location of organelles.
P. embryolabi sperm differs in the location of the acrosome, in the presence of a collar around the base of the
flagellum, and due to the close attachment of the flagellum to the non-flagellar part of the cell. Due to this
attachment, a mature P. embryolabi spermatozoon is probably able become an undulating cell capable of
movement in the densely packed inner space of an animal. The filiform shape of the mature sperm is likely
correlated with the specificity of the P. embryolabi reproductive strategy, i.e. viviparity of larvae, when thousands
of embryos, larvae, germ cells, and cells of vasoperitoneal tissue occupy the body cavity; thus, the spermatozoon
has to squeeze in narrow spaces.